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G 群链球菌上的 M 蛋白与 A 群链球菌上的 M 蛋白的生物学及免疫化学特性一致性

Biological and immunochemical identity of M protein on group G streptococci with M protein on group A streptococci.

作者信息

Jones K F, Fischetti V A

出版信息

Infect Immun. 1987 Mar;55(3):502-6. doi: 10.1128/iai.55.3.502-506.1987.

DOI:10.1128/iai.55.3.502-506.1987
PMID:3546129
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC260364/
Abstract

Previous evidence for the presence of an M or M-like protein on group G streptococci has been based on the ability of these strains to survive in human blood. In addition, cross-reactions between group A and group G streptococci have been demonstrated, but they have relied either on whole bacterial cell vaccine-induced polyclonal sera or crude protein extracts of these cells. In this study two monoclonal antibodies prepared against the purified, native group A streptococcal M6 protein demonstrated a high degree of cross-reactivity with group G streptococcal clinical isolates (9 and 19 of 22 strains examined, respectively). Ten of these strains exhibited resistance to phagocytosis when rotated in human blood. In addition, immunoblot analysis of crude mutanolysin extracts of group G streptococci with one of the M6 monoclonal antibodies illustrated a remarkable similarity in the protein pattern of these extracts as compared with those of group A streptococcal M protein. The immunoblots further demonstrated a variation in the relative molecular weights of the extracted proteins from strain to strain over a range of 57,000 to 77,000. In addition, a purified, pepsin-derived fragment (Mr, 43,000) from a group G strain was capable of eliciting rabbit antibodies that were opsonic for group G cells in a bactericidal assay. These functional and immunochemical data, in concert with DNA hybridization between group G streptococcal DNA and a group A M6 gene probe (J. R. Scott, W. M. Pulliam, S. K. Hollingshead, and V. A. Fischetti, Proc. Natl. Acad. Sci. USA 82:1822-1826, 1985), provide strong evidence for the presence of an M protein on these organisms and indicate its probable role as a virulence molecule on the surface of group G streptococci.

摘要

先前关于G群链球菌上存在M或M样蛋白的证据是基于这些菌株在人血液中存活的能力。此外,已证实A群和G群链球菌之间存在交叉反应,但这些反应要么依赖于全细菌细胞疫苗诱导的多克隆血清,要么依赖于这些细胞的粗蛋白提取物。在本研究中,针对纯化的天然A群链球菌M6蛋白制备的两种单克隆抗体与G群链球菌临床分离株表现出高度交叉反应(分别在检测的22株菌株中有9株和19株)。其中10株菌株在人血液中旋转时表现出抗吞噬作用。此外,用其中一种M6单克隆抗体对G群链球菌的变溶菌素粗提取物进行免疫印迹分析表明,与A群链球菌M蛋白提取物相比,这些提取物的蛋白模式具有显著相似性。免疫印迹进一步证明,不同菌株提取蛋白的相对分子量在57,000至77,000范围内存在差异。此外,来自G群菌株的一种纯化的、胃蛋白酶衍生片段(Mr,43,000)能够引发兔抗体,这些抗体在杀菌试验中对G群细胞具有调理作用。这些功能和免疫化学数据,与G群链球菌DNA和A群M6基因探针之间的DNA杂交结果(J. R. Scott、W. M. Pulliam、S. K. Hollingshead和V. A. Fischetti,《美国国家科学院院刊》82:1822 - 1826,1985)相结合,为这些生物体上存在M蛋白提供了有力证据,并表明其可能作为G群链球菌表面的毒力分子发挥作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41f7/260364/6b6edc864529/iai00087-0016-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41f7/260364/8a52b5ce9e90/iai00087-0016-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41f7/260364/6b6edc864529/iai00087-0016-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41f7/260364/8a52b5ce9e90/iai00087-0016-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41f7/260364/6b6edc864529/iai00087-0016-b.jpg

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